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Functional roles for the GerE-family carboxyl-terminal domains of nitrate response regulators NarL and NarP of Escherichia coli K-12

机译:Gere-Family羧基末端结构域的功能作用硝酸盐响应调节剂NARL和大肠杆菌K-12的NARP

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NarL and NarP are paralogous response regulators that control anaerobic gene expression in response to the favoured electron acceptors nitrate and nitrite. Their DNA-binding carboxyl termini are in the widespread GerE–LuxR–FixJ subfamily of tetrahelical helix–turn–helix domains. Previous biochemical and crystallographic studies with NarL suggest that dimerization and DNA binding by the carboxyl-terminal domain (CTD) is inhibited by the unphosphorylated amino-terminal receiver domain. We report here that NarL-CTD and NarP-CTD, liberated from their receiver domains, activated transcription in vivo from the class II napF and yeaR operon control regions, but failed to activate from the class I narG and fdnG operon control regions. Alanine substitutions were made to examine requirements for residues in the NarL DNA recognition helix. Substitutions for Val-189 and Arg-192 blocked DNA binding as assayed both in vivo and in vitro, whereas substitution for Arg-188 had a strong effect only in vivo. Similar results were obtained with the corresponding residues in NarP. Finally, Ala substitutions identified residues within the NarL CTD as important for transcription activation. Overall, results are congruent with those obtained for other GerE-family members, including GerE, TraR, LuxR and FixJ.
机译:Nar1和Narp是递质的副骨反应调节剂,其控制厌氧基因表达响应于有利的电子受体硝酸盐和亚硝酸盐。它们的DNA结合羧基末端是四螺旋螺旋螺旋域的广泛的Gere-Luxr-FixJ亚家族。与Nar1的先前生化和晶体研究表明,由不磷酸化的氨基末端接收器域抑制羧基 - 末端结构域(CTD)的二聚化和DNA结合。我们在此报告,NARL-CTD和NARP-CTD,从其接收方框中解放,从II级NAPF和年度操纵子控制区域中激活了VIVO的转录,但未能从I类NARG和FDNG操纵控区域激活。进行丙氨酸取代以检查NARL DNA识别螺旋中残留物的要求。 Val-189的取代和Arg-192阻断的DNA结合在体内和体外测定,而Arg-188的取代仅在体内具有很强的效果。在NARP中的相应残留物获得了类似的结果。最后,ALA取代鉴定了NARL CTD内的残留物对转录激活。总体而言,结果与其他Gere-Family成员获得的结果一致,包括Gere,Trar,Luxr和FixJ。

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